A method of immunomodulation by contacting the bodily fluid of a patient with renal tubule cells outside of the kidney.
|
1. A method of modulating the levels of at least one inflammatory cytokine in a patient in need thereof, comprising:
contacting, outside of the kidney, at least a portion of the body fluid of the patient with renal tubule cells, wherein the patient in need thereof is suffering from one or more disease selected from the group consisting of, malnutrition, chronic congestive heart failure, inflammatory bowel disease, Crohn's disease, ulcerative colitis, rheumatoid arthritis, ankylosing spondylitis, systemic vasculitis, lupus, Wegener's granulomatosis, polyarteritis nodosa, dermatomyositis, diabetes mellitus Type I, thyroiditis, psoriasis, Guillian barre syndrome, multiple sclerosis, and atherosclerosis, or other autoimmune disorders.
2. The method of
3. The method of
4. The method of
5. The method of
|
1. Field of the Invention
The present invention relates to a method for modulating inflammatory and pro-inflammatory states in a patient in need thereof by contacting the bodily fluid of the patient with renal tubule cells outside of the kidney.
2. Discussion of the Background
It is widely recognized that inflammatory cytokines play a role in the etiology of a variety of disease states, such as malnutrition, chronic congestive heart failure, inflammatory bowel disease, Crohn's disease, ulcerative colitis, rheumatoid arthritis, ankylosing spondylitis, systemic vasculitis, lupus, Wegener's granulomatosis, polyarteritis nodosa, dermatomyositis, diabetes mellitus Type I, thyroiditis, psoriasis, Guillian Barre syndrome, multiple sclerosis, and atherosclerosis, or other autoimmune disorders. [Refs. 1, 20, 21, 22, 23, 24, 25, 31, 32, 33, 34, 35, 36, 37, 38, 39]. Modulating the levels of such cytokines may provide a method of treating such patients. Accordingly, there remains a critical need for novel inflammation modulatory therapies for the treatment of patients suffering from, for example, at least one of the diseases discussed above.
Although maintenance dialysis therapy for end-stage renal disease (ESRD) has been used for almost 40 years, annual mortality rates among patients with ESRD undergoing hemodialysis remain greater than 20%. [Refs. 1, 2]. The most common cause of death in end-stage in ESRD patients (about 50%) is of cardiac or cardiovascular origin, with infection/sepsis (about 15%) being second. [Ref. 1].
The mortality from sepsis complicated by renal failure remains extremely high despite the application of modern renal replacement therapy. The systemic inflammatory response syndrome, or SIRS, is a catastrophic sequela of a variety of clinical insults, including infection, pancreatitis and cardiopulmonary bypass, and claims over a quarter million lives in the United States each year. [Refs. 3, 4, 5, 6, 7, 8].
The mortality is especially high in patients with multiple system organ failure syndrome (MSOF) and acute renal failure (ARF). The excess mortality seen in patients with sepsis and ARF is not ameliorated by conventional renal replacement therapy, which treats volume overload, uremia, acidosis, and electrolyte derangements. [Refs. 9, 6].
The prevalence of inflammation is high in dialysis patients; several lines of evidence suggest the presence of an ongoing acute-phase reaction in patients with ESRD undergoing hemodialysis. [Refs. 10, 11, 12]. Blood monocytes from hemodialysis patients are primed for cytokine production and predialysis serum contains elevated concentrations of inflammatory cytokines (for example, tumor necrosis factor-alpha [TNF-α], interleukin-beta [IL-1β], interleukin-1, [IL-1], interleukin-6 [IL-6], interleukin-8 [IL-8], lipopolysaccharide biding protein, soluble lipopolysaccharide receptors [CD-14], GM-CSF, G-CSF, and chemokines) and anti-inflammatory cytokines (soluble TNF receptors [TNF-RI and TNF-RII], interleukin receptor antagonist [IL-1ra], interleukin-4 [IL-4], interleukin-10 [IL-10], interleukin-12 [IL-12], interleukin-13 [IL-13], and transforming growth factor-β [TGF-β]). [Refs. 13, 14, 15, 16, 17, 30].
In fact, one of the strongest independent risk factors of mortality among patients undergoing hemodialysis is hypoalbuminemia. [Refs. 18, 19]. The generation of albumin is reduced and hypoalbuminemia develops as part of the acute phase response, mediated by proinflammatory cytokines (most directly interleukin-6 [IL-6]). [Ref. 2]. Accordingly, there remains an ongoing need for new methods for modulating the inflammatory response among hemodialysis patients.
It is an object of the present invention to provide methods of modulating the levels of at least one inflammatory cytokine in a patient in need thereof.
It is another object of the present invention to provide methods for increasing the level of at least one inflammatory cytokine in the patient.
It is another object of the present invention to provide methods for decreasing the level of at least one inflammatory cytokine in the patient.
It is another object of the present invention to provide methods of treating hemodialysis patients suffering from ESRD, chronic renal insufficiency (CRI), SIRS, ARF, or sepsis by modulating the inflammatory response, by modulating the levels of inflammatory cytokines.
It is another object of the present invention to provide methods of treating non-renal diseases which are associated with a suppressed or stimulated inflammatory response. These diseases include malnutrition, chronic congestive heart failure, inflammatory bowel disease, Crohn's disease, ulcerative colitis, rheumatoid arthritis, ankylosing spondylitis, systemic vasculitis, lupus, Wegener's granulomatosis, polyarteritis nodosa, dermatomyositis, diabetes mellitus Type I, thyroiditis, psoriasis, Guillian Barre syndrome, multiple sclerosis, and atherosclerosis.
The present invention is based, in part, on the discovery that modulation of inflammatory cytokines can be used to treat a patient in an acute or chronic inflammatory state. Such a patient may be suffering from ESRD, chronic renal insufficiency (CRI), SIRS, ARF, or sepsis. This treatment method includes contacting a body fluid with renal tubule cells outside of the kidney As a result of this contact, the tubule cells introduce mediators into and/or reabsorb mediators from the body fluid. After contact with the tubule cells, at least a portion of the body fluid is recirculated to the patient, where the presence of mediators introduced to the body fluid or the absence of mediators due to reabsorption induce a response in the patient, which leads to amelioration of the inflammatory state by modulation of the inflammatory cytokines.
Accordingly, the objects of the present invention, and others, may be accomplished with a method of treating a patient in an acute or chronic inflammatory state by modulating the levels of the inflammatory cytokines, comprising:
contacting, outside of the kidney, at least a portion of a body fluid of the patient with renal tubule cells.
The objects of the present invention, and others, may also be accomplished with a method of treating a patient in an acute inflammatory state by modulating the levels of the inflammatory cytokines, comprising:
removing a portion of body fluid from the patient,
contacting the removed body fluid with renal tubule cells, and
returning at least a portion of the body fluid, which has been, contacted with the renal tubule cells to the patient.
The objects of the present invention may also be achieved by enhancing at least one inflammatory cytokine, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
The objects of the invention may also be achieved by suppressing at least one inflammatory cytokine, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
In this respect, examples of proinflammatory cytokines include tumor necrosis factor-alpha [TNF-α], interleukin-beta [IL-1β], interleukin-1, [IL-1], interleukin-6 [IL-6], interleukin-8 [IL-8], lipopolysaccharide-biding protein, soluble lipopolysaccharide receptors [CD-14], GM-CSF, G-CSF, and chemokines.
In this respect, examples of anti-inflammatory cytokines include soluble TNF receptors [TNF-RI and TNF-RII], interleukin receptor antagonist [IL-1ra], interleukin-4 [IL-4], interleukin-10 [IL-10], interleukin-12 [IL-12], interleukin-13 [IL-13], and transforming growth factor-β [TGF-β].
In a preferred embodiment, the above-stated objects may be obtained by contacting the body fluid with the renal tubule cells ex vivo.
Another embodiment of the present invention involves contacting the body fluid with the renal tubule cells inside the body of the patient.
A preferred embodiment of the present invention is the enhancement of at least one inflammatory cytokine by contacting a body fluid with renal tubule cells outside of the kidney, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
In another embodiment of the present invention, at least one inflammatory cytokine may be suppressed by contacting a body fluid with renal tubule cells outside of the kidney, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
The above objects highlight certain aspects of the invention. Additional objects, aspects and embodiments of the invention are found in the following detailed description of the invention.
A more complete appreciation of the invention and many of the attendant advantages thereof will be readily obtained as the same becomes better understood by reference to the following Figures in conjunction with the detailed description below.
Unless specifically defined, all technical and scientific terms used herein have the same meaning as commonly understood by a skilled artisan in biochemistry, cellular biology, molecular biology, and the medical sciences.
All methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, with suitable methods and materials being described herein. All publications, patent applications, patents, and other references mentioned herein are incorporated by reference in their entirety. In case of conflict, the present specification, including definitions, will control. Further, the materials, methods, and examples are illustrative only and are not intended to be limiting, unless otherwise specified.
The present invention is based, in part, on the discovery that modulation of inflammatory cytokines can be used to treat a patient in an inflammatory state. Such a patient may be suffering from ESRD, chronic renal insufficiency (CRI), SIRS, ARF, or sepsis. A further description of SIRS is provided by U.S. patent application Ser. No. 09/941,987 filed Aug. 30, 2001, which is incorporated herein by reference in its entirety.
This treatment method includes contacting a body fluid with renal tubule cells outside of the kidney. Without being limited to any particular theory, it is believed that as a result of this contact, the tubule cells introduce mediators into the body fluid and/or reabsorb mediators from the body fluid. After contact with the tubule cells, at least a portion of the body fluid is recirculated to the patient, where the presence of mediators introduced to the body fluid or the absence of mediators due to reabsorption induce a response in the patient, which leads to amelioration of the inflammatory state by modulation of the inflammatory cytokines.
As will be readily appreciated by one skilled in the art, the renal disorders ESRD, chronic renal insufficiency (CRI), SIRS, ARF, or sepsis differ in their etiology, individual cytokine response, and treatment regimen. However, these disorders share a relationship involving a acute inflammatory state. Accordingly, a method of modulating the cytokine response levels thereby ameliorating the associated disorder would be of tremendous importance in the medical field.
However, the need for modulating the levels of inflammatory cytokines is not limited to patients on hemodialysis or suffering a renal ailment. It has been widely recognized that inflammatory cytokines play a role in the etiology of malnutrition, chronic congestive heart failure, inflammatory bowel disease, Crohn's disease, ulcerative colitis, rheumatoid arthritis, ankylosing spondylitis, systemic vasculitis, lupus, Wegener's granulomatosis, polyarteritis nodosa, dermatomyositis, diabetes mellitus Type I, thyroiditis, psoriasis, Guillian Barre syndrome, multiple sclerosis, and atherosclerosis, as well as other autoimmune disorders. [Refs. 1, 20, 21, 22, 23, 24, 25, 31, 32, 33, 34, 35, 36, 37, 38, 39].
The inventor has discovered that an element of amelioration of the aforementioned disorders is that when the body fluid is contacted with the renal tubule cells, the cytokine response and hemodynamics of animals are affected. Accordingly, the renal tubule cells provide an immunomodulatory effect. This effect is most notably achieved by modulating inflammatory cytokine expression, either by stimulating or suppressing expression thereof.
The inventive method involves contacting, outside of the kidney, at least a portion of the body fluid of the patient with renal tubule cells. A preferred embodiment of the present invention is the enhancement of at least one inflammatory cytokine by contacting a body fluid with renal tubule cells outside of the kidney, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
In another embodiment of the present invention, at least one inflammatory cytokine may be suppressed by contacting a body fluid with renal tubule cells outside of the kidney, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
In another embodiment of the invention, the object of modulating the levels of inflammatory cytokines can be achieved by removing a portion of body fluid from the patient, then contacting the removed body fluid with renal tubule cells, and subsequently returning at least a portion of the body fluid which has been contacted with the renal tubule cells to the patient.
The method of the present invention may provide for enhancing the levels of at least one inflammatory cytokine, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine. Alternatively, the method of the present invention may provide for suppressing the levels of at least one inflammatory cytokine, where the inflammatory cytokine may be either a proinflammatory cytokine or an anti-inflammatory cytokine.
Known examples of proinflammatory cytokines include, but are not limited to, tumor necrosis factor-alpha [TNF-α], interleukin-beta [IL-1β], interleukin-1, [IL-1], interleukin-6 [IL-6], interleukin-8 [IL-8], lipopolysaccharide-biding protein, soluble lipopolysaccharide receptors [CD-14], GM-CSF, G-CSF, and chemokines.
Known examples of anti-inflammatory cytokines include, but are not limited to, soluble TNF receptors [TNF-RI and TNF-RII], interleukin receptor antagonist [IL-1ra], interleukin-4 [IL-4], interleukin-10 [IL-10], interleukin-12 [IL-12], interleukin-13 [IL-13 ], and transforming growth factor-β [TGF-β].
Modulation of inflammatory cytokines can be assessed by determining the level (reported in pg/ml) of each cytokine in the plasma or by measuring the level of expression of the cytokines in the blood cells. Plasma cytokine levels can be determined, for example, by utilizing a cytokine detection kit. One such kit is manufactured and distributed by R & D Systems, Inc. (Minneapolis, Minn.). Expression levels of cytokine genes in the blood cells may be determined, for example, by microarray analysis. One skilled in the art may find technical guidance for microarray techniques in the recent review by John Quackenbush [Ref. 40].
The patient may be a human or a non-human animal, such as a mammal. Exemplary non-human animals include dogs, cats, horses, cows, sheep, goats, and pigs. Human patients are especially preferred.
A feature of the present invention is that the body fluid of the patient is contacted with renal tubule cells. It is important to note that the body fluid of the patient is contacted with renal tubule cells outside of the kidney. In the present invention, the natural flow of the body fluid is interrupted so that the fluid can interact with the renal tubule cells. After this contact, the body fluid is returned to the course of natural flow in the patient's body. Thus, the present invention is distinct from the natural physiological processes, which occur in the kidney.
Methods and devices for contacting a body fluid with renal tubule cells and then returning the treated fluid to the patient are well known in the art. See, for example, references 26, 27, 28, 29, and U.S. Pat. No. 6,150,164, all of which are incorporated herein by reference in their entirety. In a particularly preferred embodiment of the invention, the body fluid of the patient is contacted in with the renal tubule cells in a renal tubule assist device (RAD). As used herein, the term “renal tubule assist device” refers to a device, which contains (1) renal tubule cells and (2), an inlet and outlet for the body fluid, where the body fluid is contacted with the renal tubule cells inside the device. Such a device is described in detail in the publications cited immediately above. An example of a suitable RAD is shown in
In addition to the methods described in the publications cited immediately above, the renal tubule cells may also be grown on solid or porous microcarrier beads. Examples of suitable microcarrier beads include micropourous gelatin and collagen-coated dextran. In this embodiment, the cells can be grown on the beads. Then, the cells can be detached from the beads and be seeded in the RAD. In another embodiment, the cells on the beads can be used in the extracapillary space of a sepsis-treating cartridge on microcarrier beads as opposed to single monolayers along the inner surface of hollow fibers. Thus, a body fluid of a patient could be perfused into a cartridge containing these cells in this formulation for exposure to the patient's fluid and respond with mediators that would modulate the levels of the inflammatory cytokines.
The tubule cells may be obtained from a human or a non-human animal source. The non-human animal is preferably a mammal. Suitable examples of non-human cells are porcine, rat, dog, mouse, or rabbit tubule cells. Transformed tubule cells may also be used in the present invention. Such cells are described in, for example, U.S. Pat. No. 6,150,164.
The body fluid may be blood, plasma, or ultrafiltrate of plasma. Venous blood is particularly preferred. Arterial blood may also be used.
In one embodiment of the invention, the body fluid of the patient is contacted in with the renal tubule cells ex vivo, i.e, outside of the body of the patient. In an alternative embodiment, the body fluid is contacted in with the renal tubule cells inside the body of the patient.
In one embodiment, the renal tubule assist device is ex vivo. Alternatively, the renal tubule assist device is implanted in the patient.
In another embodiment, the implanted renal tubule cells may be contained within a cell cartridge, which may be implanted into an intact blood vessel. An example of a device that can be implanted is described in, for example, U.S. Pat. No. 5,704,910 and U.S. Pat. No. 5,911,704, the entire contents of both of these patents are incorporated herein by reference in their entirety.
The patient may also be afflicted with renal disease, for example acute renal failure or chronic renal failure. Such a patient may be afflicted with end-stage renal disease. The patient may also be septic. Such a patient may also be on hemo- or peritoneal dialysis. Further, the patient may be suffering from malnutrition, chronic congestive heart failure, inflammatory bowel disease, Crohn's disease, ulcerative colitis, rheumatoid arthritis, ankylosing spondylitis, systemic vasculitis, lupus, Wegener's granulomatosis, polyarteritis nodosa, dermatomyositis, diabetes mellitus Type I, thyroiditis, psoriasis, Guillian Barre syndrome, multiple sclerosis, and atherosclerosis.
An example of a specific embodiment of the present invention is shown in
Having generally described this invention, a further understanding can be obtained by reference to certain specific examples, which are provided herein for purposes of illustration only, and are not intended to be limiting unless otherwise specified.
A 29 year-old man presented to the emergency room with a one-day history of nausea, vomiting, diarrhea, chills and fever. The morning of admission he noted redness, swelling and pain in his right thigh. Over the subsequent four hours the redness, swelling and pain extended to his calf. Upon presentation, the patient had a temperature of 103.5° F., and blood pressure of 101/42. Bibasilar rates were noted. His right thigh and calf were erythematous, swollen and tender. On admission, his white blood count was 20,200 with a marked left shift, and his platelet count was 174,000. His serum electrolytes were normal, but his serum creatinine was 2.9 mg/dl and BUN 38 mg/dl. His arterial blood gases on 3 L nasal cannula was pH 7.46 pCO2 32 mm Hg, pO2 65 mm Hg. Chest x-ray showed no infiltrates. Blood cultures were obtained, ceftriaxone 2 gm and clindamycin 900 mg were given intravenously. A CT scan of his right leg revealed no gas, fluid collections or necrotizing tissue.
After slight improvement over the first 24 hours, his condition began to rapidly deteriorate with shortness of breath, oliguria and hypotension. Repeat plasma chemistry values revealed rising liver function tests with alanine amino transferase (ALT) 155 IU/1, aspartate amino transferase (AST) 189 IU/1, total bilirubin 4.1 mg/dl, serum creatinine 7.6 mg/dl, BUN 69 mg/dl, calcium 6.8 mg/dl and a creatinine phosphokinase 460 IU/1. Arterial blood gases on 6 L nasal cannula were pH 7.23, pCO2 40 mm Hg, pO2 68 mm Hg. Chest x-ray revealed multilobar infiltrates. A clinical diagnosis of streptococcal toxic shock syndrome was made and intravenous antibiotics were continued with ceftriaxone 2 gm q8h, clindamycin 900 mg q8h and a single dose of vancomycin, 1.5 gm. He was transferred to the intensive care unit approximately 24 hours after admission and intubated to maintain adequate oxygenation attaining a pO2 of 68 mm Hg with FiO2 of 60 percent. His blood cultures were reported positive for beta hemolytic streptococcus Group A. Emergent surgical exploration of his left calf revealed no necrotizing fasciitis or myonecrosis, which was confirmed on histologic evaluation. Tissue specimens from the procedure were also culture positive for beta-hemolytic streptococcus Group A.
After returning from surgery, now 36 hours after admission, his condition continued to deteriorate with worsening hypotension to 68/42 requiring vasopressor support with dopamine, phenylephrine, and levarterenol. He was started on continuous venovenous hemofiltration to treat his acute renal failure. Over the subsequent 72 hours, his liver function tests elevated to a high of ALT 904, AST 1404, total bilirubin 5.6 mg/dl, creatinine phosphokinase 45,530, and lows of serum calcium 5.9 mg/dl, serum albumin 1.8 mg/dl, hematocrit 29.5 percent, platelet count 28,000. During this critical period, his cardiac output was markedly elevated between 9-12 L/min and his systemic vascular resistance varied between 300-500.
Because of his worsening condition, the patient was considered to be included in a Phase I/II clinical trial at The University of Michigan to test the safety and functionality of a bioartificial kidney. Pre-clinical large animal experiments have suggested that this device can ameliorate the cardiovascular consequences of septic shock in uremic animals. This study is an investigator-initiated trial reviewed and approved by the U.S. Food and Drug Administration (FDA) and be the local institutional review board (IRB). The patient met all inclusion and exclusion criteria of the protocol and his family agreed to allow him to participate in the study and signed a detailed informed consent document.
The bioartificial kidney is comprised of a continuous venovenous hemofiltration (CVVH) circuit connected to a synthetic hemofiltration cartridge, and a Renal Tubule Assist Device (RAD). The RAD is a commercial hemofiltration cartridge (Fresenius F40, Fresenius AG, Bad Hamburg, Germany) in which human renal tubule cells have been grown to confluence along the inner surface of the hollow fibers. The human cells were isolated and expanded from human kidneys obtained from the National Disease Research Interchange (NDRI, Arlington, Va., USA). NDRI is a not-for-profit organization and provides tissues and organs originally retrieved for transplant, but due to donor/recipient incompatibility, transplantation is not possible. A written informed consent document was obtained for each kidney donor and is kept on file at the tissue acquisition site.
After 36 hours of CVVH, the bioartificial kidney replaced the hemofiltration cartridge in the extracorporeal circuit. A variety of physiologic parameters of the patient were carefully monitored prior to, during and after the use of the biohybrid device. Key parameters are summarized in
As displayed in
Key physiologic parameters, which contributed to the improved Apache 3 predicted mortality rates, are summarized in
The effect on renal function was also striking. As seen in
In addition, the 21.5 hours of treatment coincided with a reduction in plasma creatinine concentrations from 7.0 mg/dl to 6.0 mg/dl despite ongoing rhabdomyolysis as reflected with the elevated CPKs during this treatment interval. In fact, both plasma and urine myoglobin levels were greater than 100,000 ng/ml during this treatment period.
The RAD also demonstrated maintenance of excellent viability and functionality during the treatment period. Renal tubule cell counts exiting the RAD in the processed ultrafiltrate was over the treatment interval cumulatively less than 0.1% of the total renal epithelial cell number (approximately 1.0×109 cells) within the device. This maintained viability occurred during treatment of a critically ill uremic individual with toxic shock syndrome and marked myoglobinuria. The functionality of tubular cell function was demonstrated by the tubular fluid/ultrafiltrate glutathione (GSH) ratios, which averaged 0.72 demonstrating active breakdown and transport of amino acids by the tubule cells. Plasma 1,25-dihydroxy-vitamin D3 levels also improved during the treatment interval from 15 pg/ml to 22 pg/ml (normal range=17 pg/ml to 53 pg/ml), demonstrating endocrinologic activity of the cells.
Fortunately for the patient, despite an Apache 3 score predicting as high as a 92 percent in-hospital mortality rate, he eventually improved with his liver function tests returning to normal, respiratory parameters improving with successful extubation, and a return to normal renal function, so that hemofiltration and hemodialysis was discontinued. He was discharged from the ICU after 13 days and the acute care hospital after 20 days.
The mechanism by which renal tubule cells may have affected these physiological parameters of this patient may be related to a possible role the kidney plays in immunomodulation during stress states, as suggested by preclinical large animal experiments performed by the inventor.
In this regard, plasma cytokine levels were measured in this patient prior to, during, and post-RAD therapy. Blood from the patient was collected into tubes containing sodium heparin as the anticoagulant. These tubes are immediately taken to the laboratory where they were centrifuged for 5-10 minutes at 3500 rpm to separate the blood plasma from its cellular components. The plasma was then separated into small aliquots. These aliquots were quickly frozen using liquid nitrogen before being stored at −70° C.
The cytokine assays employed a quantitative sandwich enzyme immunoassay technique. An antibody specific for the cytokine of interest was pre-coated into strips of microtiter wells by the assay kit manufacturer (R & D Systems, Inc., Minneapolis, Minn.). Technicians begin by pipetting standards with known concentrations and patient plasma samples into the wells. Any cytokine present in the plasma was bound to the wells by the immobilized antibody. After washing away unbound substances, an enzyme-linked antibody specific for the cytokine was added to the wells. Another wash was performed to remove any unbound antibody-enzyme reagent. Next, a substrate solution was added to the wells and color develops in proportion to the amount of cytokine which was bound in the initial step. The color development was then stopped and the intensity of the color was measured. Plasma cytokine concentrations were then calculated according to the color measurements of the known concentrations of the standards.
As demonstrated in Table 1 and
TABLE 1
Plasma Levels of Inflammatory Proteins with RAD Therapy; Patient from Example 1.
Normal
Time (hours)
Protein
Range
0
4
8
12
16
20
21.5
25.5
TNF-α
<15.6
20
20
21
19
14
14
11
15
(pg/ml)
STNFRI
500-2000
24,101
24,769
25,056
28,445
25,470
22,828
—
27,188
(pg/ml)
STNFRII
950-2500
50,869
53,150
47,158
—
51,139
49,091
—
44,175
(pg/ml)
IL-1β
<3.9
3
1
8
13
8
3
0
1.5
(pg/ml)
IL-lra
50-1400
17,119
10,364
7,237
2,508
7,948
8,710
10,248
6,441
(pg/ml)
IL-lsRII
2-9
103
105
94
86
—
—
95
81
(ng/ml)
IFN-•
<15.6
42
65
35
—
49
26
—
5
(pg/ml)
IL-6
<3.13
833
736
853
—
1,255
784
—
932
(pg/ml)
IL-8
<31.2
152
141
132
134
—
—
140
74
(pg/ml)
MCP-1
113-340
4,061
2,886
2,614
2,448
1,343
816
671
343
(pg/ml)
MCP-1•
<46.9
<46.9
<46.9
<46.9
<46.9
—
—
<46.9
<46.9
(pg/ml)
IL-10
<7.8
9
5
2
—
2
5
—
5
(pg/ml)
IL-13
<62.5
<125
<125
<125
<125
—
—
—
<125
(pg/ml)
G-CSF
<39
684
598
485
435
307
114
104
90
(pg/ml)
GM-CSF
<7.8
<7.8
<7.8
<7.8
<7.8
<7.8
—
—
<7.8
(pg/ml)
CRP
<2000
650,000
610,000
865,000
734,000
—
745,000
—
705,000
(ng/ml)
Footnotes for Table 1
Hours refer to 0 = pre-therapy; 4, 8, 12, 20 of RAD therapy; 21.5 just prior to treatment discontinuation; 25.5 is 4 hours post therapy.
Blanks identify measurements not done due to sample size limitations.
Normal values are derived from derived from diagnostic kits.
Abbreviations: TNF (tumor necrosis factor)-α; STNFR (soluble TNF receptor)-I, II; IL (interleukin)-1β; IL-lra (receptor antagonist); IL-lsr (soluble receptor)-II; IFN (interferon)-•; MCP (monocyte chemoattractant protein)-1; MIP (macrophage migratory inhibitory factor)-I•; G (granulocyte)-CSF (colony stimulating factor); GM (macrophage)-CSF; CRP (C-reactive protein).
A 23 year old male with no significant past medical history presented to the emergency room, versed and intubated for airway protection, for work up and management of severe metabolic acidosis and unresponsiveness. He had no known drug allergies, is not on any medicines at home. He is a nonsmoker and not an illicit drug/alcohol user per family. Further, there is no history of depression or recent travel. Prior to presentation, the patient complained of abdominal pain, nausea and vomited once. The nausea and vomiting persisted for several hours. The patient was found unresponsive in a pool of vomitus.
In the emergency room, he was unconscious, afebrile, hemodynamically stable with a blood pressure (BP) of 130/80 mm of Hg and a heart rate (HR) of 90-bpm. The patient's respiratory rate was 20/min and 94% sat. Except for unresponsiveness, the examination was unremarkable with a Glasgow coma scale of 2. Initial blood work showed severe metabolic acidosis with bicarbonate of 9 mmol/l, high anion gap of 23, potassium of 7.7 mmol/l and serum creatinine of 1.1 mg/dl. ABG 7.17/19/123/7/99%. The lactic acid level was 9.3 mmol/l. CBC revealed a white blood cell (WBC) count of 12.3, hemoglobin (Hb) of 17.3 with 52.6 hematocrit (Hct) and 300 platelets. Lumbar puncture was performed and cerebral spinal fluid (CSF) showed no red blood cells (RBC), 1 WBC, 35 protein and 70 glucose. Gram stain was negative. CT head, abdomen and pelvis showed no acute process. Ammonia level was 79.
The patient was treated with intravenous fluid (IV), 6 amps of sodium bicarbonate and Ceftriaxone 2 grams IV. A gram of Phenytoin was given for twitching.
In the ICU, he was on the ventilator, with 135/70 BP and 97 bpm HR. Pupils were normal in size, reacting to light and the gag reflex was present. Reflexes were normal. The lungs were clear to auscultation bilaterally. Heart rate was regular without murmurs, rub or gallop. The abdomen was soft, nontender without hepatosplenomegaly. Bowel sounds were present. There was no peripheral edema. Occasional myoclonus was noted. No skin rash or petechie was seen.
Labs were as follows:
At 3:50 PM on the day of admission, 154 mmol/l Na, 4.8 mmol/l K, 111 mmol/l Cl, 9 mmol/l HCO3, 16 mg/dl BUN, 2.2 mg/dl Cr. AG of 35. 8.7 mg/dl Ca, 6.5 mg/dl Ph, 1.9 mg/dl Mg, 6.6 g/dl T.pr, 4.1 g/dl Alb, 13 U/l AST, 82 U/l ALT, 0.4 mg/dl Bil, 12.9 PT/1.13 INR, 30.7 PTT, 17.37 WBC, 14 gms Hb, 42 HCT, 228 Plt. 11 ESR, 0.8 mg/dl CRP, 175 CPK with 5.2 MB. Osmolal gap was 5 (326-321). ABG 7.21/21/587/8/98/100% on 100% FiO2. 10 mmol/l lactic acid. Urine analysis showed few RBC, few WBC, 2+ protein and lots of calcium oxalate crystals. No cellular casts were seen.
Serum and urine toxicology screen was negative for acetominophen, ethanol, aspirin, tricyclic acids, opiates and cocaine. Benzodiazepines were positive in urine. Blood was sent for ethylene glycol levels. EKG showed sinus rhythm with right axis deviation and poor R wave progression. MRA of the brain did not show any bleeding or structural lesion.
IV fluids and bicarbonate replacement was continued. Ceftriaxone, Cipro and Vancomycin were given empirically after blood cultures were drawn.
At 6:00 PM on the day of admission, serum creatinine was 2.5 mg/dl with a urine output of 30 ml/hr. At 8:30 PM on the day of admission, serum creatinine was 2.8 mg/dl with decreasing urine output. Serum creatinine increased to 5 mg/dl with further decrease in the urine output by the following day. The patient was started on lasix and Diuril without adequate response. Renal ultrasound showed 11.3 cm left kidney and 11.9 cm right kidney without any hydronephrosis. CT abdomen without contrast showed enhancement of the renal cortex, consistent with toxic ingestion.
On the second day after admission, serum creatinine was 6.5 mg/dl with no urine output. ATN of unclear etiology was considered, left groin access was placed and hemodialysis was performed for eight hours with F70 kidney, 4 k bath, 300 ml/hr of ultrafiltration, 300 ml/hr BFR and 500 ml/min DFR. Ethylene glycol screen was reported as negative. However, due to the presence of mental status changes, metabolic acidosis with high anion gap and acute renal failure with crystalluria, ethylene glycol poisoning could not be ruled out.
On the third day after admission, after screening for inclusion and exclusion criteria of the Renal Tubule Assist Device (RAD) study, the patient's family was approached and consent was obtained. Labs were drawn and continuous venovenous hemofiltration (CVVH) was started at 8:45 PM in preparation to RAD therapy. Paganini risk modeling score was 130. Mental status improved and he was following commands by moving extremities.
On the fourth day after admission, the RAD was integrated into circuit at 8:53 AM and therapy was started at 9:18 AM by the RAD team. Under close monitoring of the clinical status, reabsorption of the ultrafiltrate was gradually increased to 50%. The patient tolerated the intervention well. ACT was checked every hour and glucose was checked every 15 minutes for an hour and then every hour while on RAD. Initial ACT was 172 and glucose was 214 mg/dl. DMP, CBC and ABG's were checked every four hours. Phosphorus, calcium, magnesium, albumin, uric acid and PTT/PT/INR were drawn every eight hours.
At 1:10 PM on the fourth day after admission, ACT was 186, hence heparin was decreased to 500 u/hr from 750 u/hr. A new catheter was placed and the CVVH system was changed in just 20 minutes, at 2:00 PM, due to poor blood flows through the original catheter. During this time the RAD was flushed with the replacement fluid. Subsequently, reabsorption was resumed at 50%.
After eight hours of RAD treatment (5:30 PM), the patient was reassessed and RAD was continued for another eight hours. At 9:50 PM, the hemofiltration system was changed in 3 minutes due to a clot in the venous trap.
At 1:30 AM on the fifth day after admission, the patient was again reassess and RAD was continued for another eight hours. At 1:35 AM, the hemofiltration system clotted again and was changed in 5 minutes. At this time, heparin was increased to 750 u/hr. At 7:45 AM lines were reversed due to a collapse of the catheter. At 9:00 AM, RAD therapy was discontinued, but CVVH was continued. During the course of the study, few IV fluid changes were made based on the glucose, calcium and bicarbonate values.
As shown in
Labs on the fifth day after admission were as follows:
142 mmol/l Na, 4.2 mmol/l K, 107 mmol/l Cl, 25 mmol/l HCO3, 41 mg/dl BUN, 5.7 mg/dl Cr, 11 mg/dl CA, 2.8 mg/dl Ph, 2.6 mg/dl Mg, 721 LDH, 73 U/l AST, 65 U/l ALT, 56 U/l GGT, 0.4 mg/dl Bil, 12.8 PT/1.12 INR, 35.4 PTT, 1.1 mmol/l lactate, 12.2 WBC, 9.1 Hb, 27.1 Hct, 78 Platelet. Liver enzyme elevation and low platelets with high LDH was thought to be due to frequent system changing from clotting. A blood transfusion was given.
After discontinuation of the study, the patient continued to be anuric. CVVH was continued for solute/volume clearances. He was extubated on the eighth day after admission. Bacterial test cultures revealed no growth, therefore antibiotics were discontinued on the ninth day after admission. In addition, on the ninth day after admission, CVVH was discontinued and IHD was initiated through permcath. The urine output gradually increased to 200 cc/day by the thirteenth day after admission. At this point the patient was discharged with dialysis three times a week, accompanied by phoslo and nephrocap tablets daily.
In addition, plasma cytokine levels were measured in this patient as described in Example 1 prior to, during, and post-RAD therapy. As demonstrated in Table 2 and
TABLE 2
Plasma Levels of Inflammatory Proteins during RAD Therapy; Patient from Example 2.
Time (hours)
Normal
Post
Protein
Range
Baseline
4
8
12
16
20
24
Therapy
G-CSF
<39
59
186
131
107
47
2
0
8
(pg/ml)
IL-lra
63-1397
2669
2263
2210
2119
2237
2263
2132
2106
(pg/ml)
IL-lsRII
8-22
14360
15660
—
19908
20514
—
24675
20081
(pg/ml)
IL-6
<12.5
874
1421
987
1242
915
726
581
158
(pg/ml)
IL-8
<31.2
42
73
38
52
69
8
20
25
(pg/ml)
IL-10
<7.8
174
241
147
174
130
105
83
60
(pg/ml)
IL-13
<62.5
60
74
49
46
46
43
63
51
(pg/ml)
IL-18
36.1-257.8
319
329
331
377
418
416
414
419
(pg/ml)
MCP-1
113-340
1506
1692
1110
1346
1808
1106
1421
1323
(pg/ml)
MIP-1α
<46.9
135
143
140
143
140
143
148
143
(pg/ml)
TNF-α
<15.6
119
109
102
104
102
93
105
102
(pg/ml)
TNF-RI
512-1739
29706
31893
34035
37724
40729
33748
40905
36907
(pg/ml)
TNF-RII
787-2145
26386
26511
29461
30689
32034
31774
30779
32258
(pg/ml)
CRP
<2
546
670
939
672
673
822
747
775
(ug/ml)
Protein C
70-140%
49
62
64
61
61
64
68
67
(pg/ml)
Footnotes for Table 2
Hours refer to Baseline = pre-therapy; 4, 8, 12, 20, 24 of RAD therapy, and post therapy.
Blanks identify measurements not done due to sample size limitations.
Normal values are derived from diagnostic kits.
In addition to determining the plasma cytokine levels, microarray analysis was performed to determine the levels of protein expression in the blood. Blood samples were drawn from the patient prior to initiation of RAD therapy (0 hours), after 8 hours and 20 hours of RAD therapy, and 4 hours after completion of RAD therapy (28 hours). The blood samples were treated with an anticoagulant and the blood cells were separated from plasma by centrifugation.
The white blood cells were lysed in TRIzol reagent (Gibco) and the RNA phase was separated by chloroform, total RNA was precipitated with isopropyl alcohol, and washed with 80% ethanol. Total RNA was further cleaned with RNeasy mini kit (Qiagen). First-strand cDNA was transcribed from total RNA using T7-(dT)24 oligomer primer and SSII reverse transcriptase at 37° C. The second strand cDNA is synthesized from first-strand cDNA using DNA ligase, DNA polymerase I and T4 DNA polymerase at 16° C. (SuperScript Choice System for cDNA synthesis kit, Gibco), and then cleaned with Phase-Locking gel. Biotin-labeled cRNA is synthesized from the double strand cDNA using T7 RNA polymerase-catalyzed in vitro transcription in the presence of biotin-labeled NTP (BioArray high yield RNA transcription labeling kit, Enzo Biochem) and then fragmented at 95° C. Biotin-labeled cRNA was heated at 99° C. for 5 min in hybridization cocktail including hybridization control (Bio B, C, D, and Cre) and hybridized with at 42° C. for 16 hrs to a GeneChip® (Affymetrix), labeled with the cDNA from blood cells. The GeneChip® was then washed with non-stringent wash buffer at 50° C. and stained with streptavidin phycoerythrin (SAPE) solution. After washing at 25° C., the GeneChip® was scanned with a laser scanner (Affymetrix). The gene expression profiles were analyzed by Affymetrix Microarray Suite and Data Mining Tool software.
A 26-year old woman was hospitalized in an outlying hospital. She initially presented with fever, myalgias, and arthralgias. Her work-up revealed anemia, leukopenia, thrombocytopenia, elevated liver enzymes, and a CT scan of the abdomen suggestive of cholecystitis. She underwent laporoscopic guided cholecystectomy 6 days prior to transfer. Her post-operative course deteriorated with fevers, acidosis, hyperkalemia, and anuira. Her serologies were positive for ANA and anti-dsDNA. A diagnosis of systemic lupus erythematosis (SLE) was made. After four days, high dose steroid treatment was initiated with an improvement of her pancytopenia. A repeat CT scan revealed ascites but no biliary leak. She was started on broad-spectrum antibiotics. Because of her worsening clinical status, she was transferred after 8 days to the University of Michigan Hospital.
Upon evaluation after transfer, her diagnosis of SLE and acute renal failure secondary to acute tubular necrosis was confirmed. She was also found to have severe pancreatitis with elevated serum lipase and amylase levels, rhabdomyolysis, hyperglycemia, and hypoxemia. She deteriorated rapidly and was transferred to the medical ICU the next day. She was started on CVVH and intubated secondary to acute respiratory distress syndrome (ARDS). Broad-spectrum antibiotics were continued. She subsequently developed profound hypocalcemia to 2 mg/dl requiring a calcium drop, hyperglycemia controlled with an insulin drip, lactic acidosis, elevated protime (INR=5.5), thrombocytopenia, elevated liver enzymes, and fungemia with Candida albicans. She was maintained on steroids and antifungal therapy begun. An emergent MRI of the abdomen confirmed the diagnosis of pancreatitis but without pancreatic necrosis.
On her fifth day in the ICU, she was enrolled into the RAD clinical trial with parent's consent. Upon initiation of RAD therapy, her blood pressure was maintained with less volume support. Within three hours of therapy, her oxygen requirements were decreased from 65% to 55% FiO2. After 8 hours, FiO2 was further reduced to 50% and 45% at 14 hours. She converted from a complete anuric state to an oliguric state with a urine volume of 142 ml over the subsequent 24 hours. Her Apache III predicted mortality rates were 57% for ICU and 81% for hospital stays upon initiation of therapy. During therapy the predicted mortality rates declined to 55% and 69%, respectively. The subsequent two days following a full 24 hour course of RAD treatment, the mortality rates were 56% and 63% (ICU), and 64% and 71% (hospital). By 8:00 AM the third day post-RAD therapy, the predicted mortality rate was 47% (ICU) and 57% (hospital).
The RAD performed well without adverse events during the entire 24 hour treatment interval. Early data demonstrated virtually no cell loss and active transport by the tubule cells during the course of treatment.
In addition, plasma cytokine levels were measured in this patient as described in Example 1 prior to, during, and post-RAD therapy. As demonstrated in Table 3 and
TABLE 3
Plasma Levels of Inflammatory Proteins during RAD Therapy; Patient from Example 3.
Time (hours)
Normal
Post
Protein
Range
Baseline
4
8
12
16
20
24
Therapy
G-CSF
<39
67
83
90
122
189
176
—
10
(pg/ml)
IL-lra
63-197
2447
2945
1297
730
833
1297
—
146
(pg/ml)
IL-lsRII
8-22
183
196
210
219
197
168
166
163
(ng/ml)
IL-6
<12.5
38
83
100
213
404
312
172
94
(pg/ml)
IL-8
<31.2
66
123
150
177
271
244
250
151
(pg/ml)
IL-10
<7.8
25
27
15
15
31
27
—
35
(pg/ml)
IL-l3
<62.5
10
5
5
10
20
30
—
20
(pg/ml)
IL-1β
<3.9
<14
<14
<14
<14
<14
<14
—
<14
(pg/ml)
MCP-1
113-340
869
2140
2720
3524
5899
4169
—
2243
(pg/ml)
MIP-1α
<46.9
5
6
6
8
7
6
—
11
(pg/ml)
TNF-α
<15.6
5
5
2
5
6
5
—
8
(pg/ml)
TNF-RI
512-1739
32105
31722
33780
35554
37289
34465
—
33316
(pg/ml)
TNF-RII
789-2145
47552
50987
53370
51653
49749
48078
—
46051
(pg/ml)
IFN-γ
<15.6
<39
<39
<39
<39
<39
<39
—
<39
(pg/ml)
Footnotes for Table 3
Hours refer to Baseline = pre-therapy; 4, 8, 12, 20, 24 of RAD therapy, and post therapy.
Blanks identify measurements not done due to sample size limitations.
Normal values are derived from diagnostic kits.
Numerous modifications and variations on the present invention are possible in light of the above teachings. It is, therefore, to be understood that within the scope of the accompanying claims, the invention may be practiced otherwise than as specifically described herein.
Patent | Priority | Assignee | Title |
10273284, | Oct 31 2006 | East Carolina University | Cytokine-based fusion proteins for treatment of immune disorders |
10363306, | Mar 31 2009 | East Carolina University | Cytokines and neuroantigens for treatment of immune disorders |
10695482, | Oct 14 2011 | SEASTAR MEDICAL, INC | Cartridge and method for increasing myocardial function |
10722637, | Jan 09 2012 | SEASTAR MEDICAL, INC | Cartridge and method for increasing myocardial function |
11118162, | Oct 15 2010 | SEASTAR MEDICAL, INC | Cytopheresis cartridges and use thereof |
11439739, | Jan 09 2012 | SeaStar Medical, Inc. | Cartridge and method for increasing myocardial function |
11866730, | Oct 15 2010 | SeaStar Medical, Inc. | Cytopheresis cartridges and use thereof |
8048419, | Feb 02 2006 | SEASTAR MEDICAL, INC | Extracorporeal cell-based therapeutic device and delivery system |
8251941, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
8409126, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
8425445, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
8425446, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods |
8425447, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
8430832, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
9029144, | Jun 18 2008 | SEASTAR MEDICAL, INC | Methods for enhanced propagation of cells |
9128093, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
9341626, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
9498566, | Aug 31 2007 | SEASTAR MEDICAL, INC | Selective cytopheresis devices and related methods thereof |
9669090, | Mar 31 2009 | East Carolina University | Cytokines and neuroantigens for treatment of immune disorders |
Patent | Priority | Assignee | Title |
3734851, | |||
4242460, | Dec 26 1978 | Cell culture device | |
4354933, | Feb 23 1981 | LESTER AMY 675 HARDING PLACE, D-11, NASHVILLE, TN 37211 | Implantable artificial kidney |
4973493, | Sep 29 1982 | Surmodics, Inc | Method of improving the biocompatibility of solid surfaces |
5002582, | Sep 29 1982 | Surmodics, Inc | Preparation of polymeric surfaces via covalently attaching polymers |
5360790, | Dec 11 1990 | The Regents of the University of Michigan | Method and formulations for the therapy of acute renal failure |
5414075, | Nov 06 1992 | Surmodics, Inc | Restrained multifunctional reagent for surface modification |
5429938, | Mar 02 1992 | University of Michigan | Methods and compositions for isolation and growth of kidney tubule stem cells, in vitro kidney tubulogenesis and ex vivo construction of renal tubules |
5437994, | Jun 15 1989 | Regents of the University of Michigan | Method for the ex vivo replication of stem cells, for the optimization of hematopoietic progenitor cell cultures, and for increasing the metabolism, GM-CSF secretion and/or IL-6 secretion of human stromal cells |
5459069, | Jun 15 1989 | The Regents of the University of Michigan | Device for maintaining and growing human stem and/or hematopoietics cells |
5499976, | Oct 05 1994 | Outboard Marine Corporation | Catheter retainer |
5516680, | Apr 18 1986 | REGENEMED, INC , A CALIFORNIA CORPORATION | Three-dimensional kidney cell and tissue culture system |
5549674, | Mar 02 1992 | REGENTS OF THE UNIVERSITY OF MICHIGAN, THE | Methods and compositions of a bioartificial kidney suitable for use in vivo or ex vivo |
5550050, | Apr 15 1994 | NEUROTECH USA, INC | Method for implanting encapsulated cells in a host |
5580697, | Jan 21 1993 | State of Oregon acting by and through the State Board of Higher | Chemical functionalization of surfaces |
5605822, | Jun 15 1989 | The Regents of the University of Michigan | Methods, compositions and devices for growing human hematopoietic cells |
5639275, | Aug 12 1993 | NEUROTECH USA, INC | Delivery of biologically active molecules using cells contained in biocompatible immunoisolatory capsules |
5653975, | Aug 12 1993 | NEUROTECH USA, INC | Compositions and methods for the delivery of biologically active molecules using cells contained in biocompatible capsules |
5656481, | Aug 12 1993 | NEUROTECH USA, INC | Compositions and methods for the delivery of biologically active molecules using cells contained in biocompatible capsules |
5661133, | Nov 12 1991 | The Regents of the University of Michigan | Expression of a protein in myocardium by injection of a gene |
5676943, | Aug 12 1993 | NEUROTECH USA, INC | Compositions and methods for the delivery of biologically active molecules using genetically altered cells contained in biocompatible immunoisolatory capsules |
5686289, | Oct 08 1993 | MICHIGAN, UNIVERSITY OF, THE | Method and compositions of a bioartificial kidney suitable for use in vivo or ex vivo |
5733727, | Nov 16 1993 | Indiana Research and Technology Corporation; Indiana University Research and Technology Corporation | Myocardial grafts and cellular compositions |
5763266, | Mar 04 1992 | The Regents of the University of Michigan | Methods, compositions and devices for maintaining and growing human stem and/or hematopoietics cells |
5773286, | Nov 17 1987 | NEUROTECH USA, INC | Inner supported biocompatible cell capsules |
5795790, | May 09 1995 | NEUROTECH USA, INC | Method for controlling proliferation and differentiation of cells encapsulated within bioartificial organs |
5833978, | Mar 16 1995 | Universite Laval | Method of in vitro preconditioning healthy donor's myoblasts before transplantation thereof in compatible patients suffering of recessive myopathies like muscular dystrophy, for improving transplantation success |
5843781, | Apr 28 1993 | The Johns Hopkins University School of Medicine | Implantable prosthetic vascular device having an adherent cell monolayer produced under shear stress |
5858653, | Sep 30 1997 | Surmodics, Inc.; Surmodics, Inc | Reagent and method for attaching target molecules to a surface |
5906817, | Apr 21 1993 | Institut Pasteur | Biocompatible implant for the expression and in vivo secretion of a therapeutic substance |
5919449, | May 30 1995 | GENVEC, INC | Porcine cardiomyocytes and their use in treatment of insufficient cardiac function |
5965125, | Oct 25 1995 | SHIRE HUMAN GENETIC THERAPIES, INC | Hybrid matrix implants and explants |
6060270, | Mar 02 1992 | MICHIGAN, UNIVERSITY OF, THE | Methods and compositions for isolation and growth of kidney tubule stem cells, in vitro kidney tubulogenesis and ex vivo construction of renal tubules |
6110209, | Aug 07 1997 | Method and paste for articular cartilage transplantation | |
6150164, | Sep 30 1996 | MICHIGAN, UNIVERSITY OF; REGENTS OF THE UNIVERSITY OF MICHIGAN, THE | Methods and compositions of a bioartificial kidney suitable for use in vivo or ex vivo |
6156304, | Dec 20 1990 | PITTSBURGH, UNIVERSITY OF, OF THE COMMONWEALTH SYSTEM OF HIGHER EDUCATION | Gene transfer for studying and treating a connective tissue of a mammalian host |
6653131, | Aug 30 2001 | MICHIGAN UNIVERSITY OF THE REGENTS OF THE | Method of treating systemic inflammatory response syndrome |
GB1479002, | |||
WO8901967, | |||
WO9100119, | |||
WO9207615, | |||
WO9317696, |
Executed on | Assignor | Assignee | Conveyance | Frame | Reel | Doc |
Feb 25 2003 | The Regents of the University of Michigan | (assignment on the face of the patent) | / | |||
Mar 11 2004 | HUMES, H DAVID | REGENTS OF THE UNIVERSITY OF MICHIGAN, THE | ASSIGNMENT OF ASSIGNORS INTEREST SEE DOCUMENT FOR DETAILS | 017889 | /0185 |
Date | Maintenance Fee Events |
Apr 30 2012 | M2551: Payment of Maintenance Fee, 4th Yr, Small Entity. |
Apr 28 2016 | M2552: Payment of Maintenance Fee, 8th Yr, Small Entity. |
Apr 08 2020 | M2553: Payment of Maintenance Fee, 12th Yr, Small Entity. |
Date | Maintenance Schedule |
Oct 28 2011 | 4 years fee payment window open |
Apr 28 2012 | 6 months grace period start (w surcharge) |
Oct 28 2012 | patent expiry (for year 4) |
Oct 28 2014 | 2 years to revive unintentionally abandoned end. (for year 4) |
Oct 28 2015 | 8 years fee payment window open |
Apr 28 2016 | 6 months grace period start (w surcharge) |
Oct 28 2016 | patent expiry (for year 8) |
Oct 28 2018 | 2 years to revive unintentionally abandoned end. (for year 8) |
Oct 28 2019 | 12 years fee payment window open |
Apr 28 2020 | 6 months grace period start (w surcharge) |
Oct 28 2020 | patent expiry (for year 12) |
Oct 28 2022 | 2 years to revive unintentionally abandoned end. (for year 12) |